A method is described for relieving and inhibiting the symptoms of inflammatory rheumatoid arthritis in mammals using cetyl myristoleate.
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1. A method of relieving and inhibiting the symptoms of inflammatory rheumatoid arthritis in mammals which comprises the oral administration to a mammal of an effective amount of cetyl myristoleate.
5. A method of relieving and inhibiting the symptoms of inflammatory rheumatoid arthritis in mammals which comprises the topical administration to a mammal of an effective amount of cetyl myristoleate.
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This application is a continuation-in-part of my copending application Ser. No. 682,540, filed May 3, 1976, now U.S. Pat. No. 4,049,824 issued Sept. 20, 1977.
The present invention relates to a method for relieving and inhibiting at least one of the symptoms of inflammatory rheumatoid arthritis in mammals by administering orally, topically or parenterally a therapeutically effective amount of cetyl myristoleate
CH3 (CH2)15 OCO(CH2)7 CH═CH(CH2)3 CH3
which may be extracted from the tissues of mice or produced synthetically. Osteoarthritis is one of the oldest and most common inflammatory diseases in mammals. It occurs at all ages. Studies show that 97% of all persons over age 60 have an arthritic condition which can be observed by X-ray. The most common symptoms of arthritis are pain, fever and inflammation, and it is the No. 1 crippling disease in man.
An object of the present invention is to provide a method for relieving and inhibiting the symptoms of inflammatory rheumatoid arthritis in mammals.
Another object of the invention is to inhibit the symptoms, such as pain, fever and inflammation associated with inflammatory rheumatoid arthritis in mammals by administering orally, topically or parenterally cetyl myristoleate extracted from the tissues of mice.
These and other objects will became apparent in the following detailed description of the invention.
It is well known that Freund's adjuvant will induce poly-arthritis in rats but not in mice. It has been common practice to test various compounds and compositions in laboratories to determine their effectiveness in relieving the symptoms of inflammatory rheumatoid arthritis by administering test compounds or compositions to rats having poly-arthritis induced previously by administering Freund's adjuvant. It was hypothesized that mice must contain some protective factor or mechanism which prevented the inducement of poly-arthritis in mice.
In accordance with the present invention a substance has been isolated from mice which, when administered to rats, essentially prevents the formation of poly-arthritis and the resultant symptoms when the rats are subsequently injected with Freund's adjuvant. The substance was isolated by extracting homogenized whole mice with methylene chloride. Upon purification of this extracted substance it was identified as cetyl myristoleate. The following example describes in greater detail the isolation of the effective substance from mice.
Seventy-nine mice totalling 2300 grams were macerated in an electric blender in batches of about eight mice, each batch being macerated in 400 ml methylene chloride. The final blend was poured into a 4 liter beaker. The blend was stirred until the methylene chloride separated, then the mixture was filtered under light suction through a large Buchner funnel containing filter paper covered by a thin layer of Filter-Cel. The resultant precipitate was washed with two 100 ml portions of methylene chloride. The combined filtrate and washings were separated from a top layer of water after which the methylene chloride was filtered again. This filtrate was concentrated in vacuo to a thin syrup of 167 grams which was treated with four parts of acetone and then left at -5°C for three days with brief stirring each day.
The mixture was filtered using Buchner filter paper with a layer of Filter-Cel and light suction. The precipitate was washed with four 25 ml portions of -5°C acetone. The combined filtrate and washings were concentrated in vacuo to a thin syrup of 121 grams. This material was dissolved in 500 ml of 20:1 legroin (20°-40°C), dry ether and chromatographed on 2500 ml 40-325 mesh ASTM silica gel in an appropriate column using the 20:1 legroin-ether mixture as eluent. One 1500 ml "blank" and then eleven 100 ml and six 200 ml fractions were collected.
Fraction Nos. 3-15 inclusive were combined and filtered in vacuo through 120 grams of Darco-X. The filtrate was concentrated in vacuo to a syrup of 0.15 gram. The Darco-X was further washed with several portions of methylene chloride. The 0.15 gram of syrup was dissolved in these washings which were concentrated in vacuo to a syrup of 0.8 gram of crude material. This was chromatographed using 350 ml of silica gel, 70-325 mesh ASTM using 40:1 carbon tetrachloride-ether as eluent.
Fraction Nos. 67-79 of 7 ml each gave 0.4 gram of material which was rechromatographed with 125 ml of silica gel using 60:1 carbon tetrachloride-ether in 2.5 ml fractions.
Fraction Nos. 117-127 gave 0.15 gram of purified syrup which proved to be principally the desired cetyl myristoleate (vmaxneat 1782 cm-1). Extensive thin-layer chromatography and frequent bioassays were used throughout to monitor the isolation and purification of the compound.
The following example describes the steps taken to identify the cetyl myristoleate product of Example I.
A mixture of 0.15 gram of the material obtained in Example I was heated with 2 ml of acetone and 3 ml of 10% sodium hydroxide solution under reflux with stirring for fourteen hours and then treated with 0.7 ml of 12 M HCl. Extractions were made with four 5 ml portions of methylene chloride followed by drying with Na2 SO4 and then evaporated with methylene chloride in vacuo. The 0.14 gram of material recovered was chromatographed on 140 ml of silica gel with methylene chloride as eluent. A 400 ml and one hundred ten 6 ml fractions were collected.
Fraction Nos. 20-55 gave 40 mg of cetyl alchohlol having a melting point of 49°-50°C after recrystallization from ethanol. The analysis calculated for C16 H34 O is
C -- 79.3%
h -- 14.1%
the analysis found was
C -- 79.2%
h -- 14.3%
fraction Nos. 89-110 produced 60 mg of a syrup which was further purified by chromotography. The resultant acid gave (vmaxneat 1712, 1722 (sh cm-1). The analysis calculated for C14 H26 O2 is
C -- 74.4%
h -- 11.6%
neut. equiv. -- 226.3
What was found is as follows:
C -- 74.1%
h -- 11.9%
neut. equiv. -- 225.5
A charge of 150 mg of cetyl alcohol, 150 mg of myristoleic acid, 50 mg of p-toluenesulfonic acid monohydrate of 20 ml of benzene were heated together under reflux conditions for four hours and then washed with a 10% sodium hydroxide solution. The benzene layer was recovered, dried and evaporated in vacuo.
This procedure produced 300 mg of a mobile oil which was identified as cetyl myristoleate (vmaxneat 1782 cm-1) (nuclear-magnetic-resonance and infrared spectoscopy).
Following the procedure set out in Example II, 150 mg of cetyl alcohol obtained in Example III and 150 mg of the acid obtained in Example II produced 300 mg of an ester (vmaxneat 1782 cm-1) which was identified by similar means with the products in Examples I and III.
Both the cetyl myristoleate extracted from the tissues of mice as described in Example I and cetyl myristoleate prepared synthetically as described in Example III have been found to be effective in relieving and inhibiting the symptoms of rheumatoid arthritis.
When administered orally the cetyl myristoleate may be administered in the pure state or preferably with known pharmaceutically acceptable vehicles or solvents such as Tracanth-Acacia, an emulphor-system such as is described in J. Pharm. Pharmacol., 25:344-345 (1973), propylene glycol or a vegetable oil such as corn or peanut oil. The relative proportions of vehicle and cetyl myristoleate are not critical. The daily dosage of cetyl myristoleate preferably ranges between about 0.05 and 0.75 gm for each 140-200 gms weight of the animal.
When administered topically the cetyl myristoleate is preferably administered with a vehicle capable of being absorbed through the surface of the skin. A preferred vehicle is dimethyl sulfoxide (DMSO). The relative proportions of vehicle and cetyl myristoleate again are not critical. The daily dosage of cetyl myristoleate administered topically preferably ranges between about 0.05 and 0.75 gm. for each 140-200 gms weight of the animal.
When administered parenterally a vehicle such as mineral oil is preferably used. Again the relative proportions of vehicle and cetyl myristoleate are not critical and the daily dosage of cetyl myristoleate is preferably between about 0.05 and 0.75 gm for each 140-200 gms weight of the animal.
The cetyl myristoleate produced both synthetically and by isolation from whole mice, respectively, were administered parenterally in mineral oil as a compatible carrier to male rats (Sprague Dawley Strain) ranging in weight between 140 and 200 grams. It is not necessary, however, that a carrier be used since cetyl myristoleate is itself an oil.
One set of rates was innoculated subcutaneously with 1.0 ml each of a mixture of mineral oil and 0.05 gm of the cetyl myristoleate. Twenty-four hours later the rats were innoculated with Bacto m. Butyricum (Disco 0640-33). A control group received only the Butyricum.
Another set of rats were given 1.0 ml each of a mixture of mineral oil containing 0.075 gm of the synthetically produced cetyl myristoleate. Two days later the rats were innoculated with Bacto m. Butyricum (Disco 0640-33). Another control group received only the Butyricum.
The rats in both control groups developed severe poly-arthritis during the following 10- to 18-day period which persisted through 32 days. All of these rats gradually lost weight.
About 70% of the first group (those treated with the material extracted from mice plus Butyricum) were completely protected from the poly-arthritis. They showed no swelling or other symptoms. The other 30% were partially protected during the 32-day period.
All of the second group (those treated with synthetically produced cetyl myristoleate plus Butyricum) were protected from the poly-arthritis and showed a steady gain in weight.
It was found that the purer the cetyl myristoleate the more dramatic were the results in protecting the rats from poly-arthritis. Also, an effective dosage of cetyl myristoleate preferably ranges between 0.05 and 0.75 gm for each 140-200 gms weight of the animal. However, doses smaller than and greater than this range will effectively relieve and inhibit the symptoms of rheumatoid arthritis such as pain, fever and inflammation.
Thus having described the invention in detail, it will be understood by those skilled in the art that certain modifications and variations may be made without departing from the spirit and scope of the invention as described herein and defined in the appended claims.
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| 11186536, | Aug 14 2015 | PHARMANUTRA S.P.A. | Cetylated fatty acids, system for the preparation thereof and use thereof |
| 5569676, | May 24 1995 | IMAGENETIX, INC | Method for the treatment of osteoarthritis |
| 6417227, | Apr 28 1999 | CG and Associates | Methods of delivery of cetyl myristoleate |
| 6677321, | Dec 09 1999 | Bruce, Levin | Methods and compositions for treatment of inflammatory disease |
| 6759062, | Feb 23 2000 | BIOSELECT INNOVATIONS, INC | Composition and method for treating the effects of diseases and maladies |
| 6787164, | Feb 23 2000 | BIOSELECT INNOVATIONS, INC | Composition and method for treating the effects of diseases and maladies |
| 6793942, | Feb 23 2000 | BIOSELECT INNOVATIONS, INC | Composition and method for treating the effects of diseases and maladies |
| 6841544, | Feb 23 2000 | BIOSELECT INNOVATIONS, INC | Composition and method for treating the effects of diseases and maladies |
| 7112578, | Nov 28 2000 | Bruce H., Levin | Methods and compositions for treatment of inflammatory disease |
| 7582670, | Dec 13 2001 | NATROGEN THERAPEUTICS INTERNATIONAL, INC | Methods of treating an inflammatory-related disease |
| 7772279, | Mar 21 2002 | BOTANOCEUTICALS, INC | Use of vegetable butter-based cetyl myristoleate for treating osteoarthritis and other musculoskeletal disease conditions and injuries |
| 7776914, | Mar 22 2004 | Imagenetix, Inc. | Esterified fatty acid composition |
| 7855223, | Jan 12 2004 | NATROGEN THERAPEUTICS INTERNATIONAL, INC | Method of treating inflammatory arthritis |
| 7943666, | Jul 24 2006 | Trinity Laboratories, Inc. | Esters of capsaicin for treating pain |
| 8147851, | May 12 2000 | Lypanosys Pte Limited | Treating eczema and/or psoriasis |
| 8258184, | Mar 21 2002 | Botanoceuticals, Inc. | Use of vegetable butter-based cetyl myristoleate for treating osteoarthritis and other musculoskeletal disease conditions and injuries |
| 8535696, | May 12 2000 | Lypanosys Pte Limited | Treating eczema and/or psoriasis |
| 8563525, | Jan 12 2004 | NATROGEN THERAPEUTICS INTERNATIONAL, INC | Methods of treating an inflammatory-related disease |
| 8586064, | May 12 2000 | Lypanosys Pte Limited | Treating eczema and/or psoriasis |
| 8765807, | Jul 24 2006 | Trinity Laboratories, Inc. | Esters of capsaicin for treating pain |
| 8815282, | Jul 15 2005 | Commercial method for production of room temperature-liquid cetyl myristoleate | |
| 8816109, | Jan 12 2009 | Council of Scientific & Industrial Research | Process for preparation of hexadecyl cis-9-tetradecenoate and hexadecyl cis-10-tetradecenoate |
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